Mechanism of enantioselective ester cleavage by histidine containing

Jun 1, 1991 - Cecilia Bombelli, Carlotta Bernardini, Gioia Elemento, Giovanna Mancini, Alessandro Sorrenti, and Claudio Villani. Journal of the Americ...
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3883

J. Org. Chem. 1991'56, 3883-3891

Mechanism of Enantioselective Ester Cleavage by Histidine-Containing Dipeptides at a Micellar Interface Marco C. Cleij,' Wiendelt Drenth,la and Roeland J. M. Nolte**lb Departments of Organic Chemistry, University at Utrecht, Utrecht, The Netherlands, and University at Nijmegen, Nijmegen, The Netherlands

Receioed January 15, 1991

Chiral p-nitrophenyl esters derived from the aniino acid phenylalanine are cleaved by histidine-containing dipeptides at a micellar interface. High enantioseledivities (up to kL/kD = 30.4 at 0 "C) are observed. Both the substratesand the catalysts contain an alternating sequence of hydrophobic and hydrophilic groups. Due to the need for hydration of the hydrophilic groups, the hydrophobic groups cannot dissolve completely into the micellar hydrocarbon phase. The kinetic data suggest that the micellar interface is capable of discriminating between transition states that have different hydrophilic and hydrophobic properties. One of the diastereomeric transition states is characterized by a hydrogen bond between the amide CO group of the ester and an NH group of the histidine-containing dipeptide. Upon formation of this hydrogen bond these polar CO and NH groups lose their hydrophilicity which allows the transfer of the adjacent apolar groups to the micellar hydrocarbon phase. The other diastereomeric transition state cannot form this hydrogen bond and the hydrophobic groups remain hydrated. Consequently,the latter transition state is of higher energy. The kinetic data reveal that it is important to prevent steric hinderance between the reactants in order to allow the unhindered formation of the hydrogen bond.

Introduction In the past 10 years an increasing number of papers has

Chart I. Catalysts H 0 I II RLC-N-C*H-C-N-C*H--COOH II I 0 H

been published dealing with reactions in aqueous surfactant solutions.* Many of these reactions occur at the micellar hydrocarbon-water interface. The adsorption of reactants at these micellar interfaces and their subsequent reaction resemble reactions that are controlled by enzymes. Large rate enhancements have been observed due to a concentration of the reactants in the micellar pseudophase.2b However, it is only until recently that high (enantio-) selectivities have been realized which are so characteristic of enzyme-controlled reactions. A number of these papers, in which remarkable enantioselectivities are reported, deal with the cleavage of chiral amino acid pnitrophenyl esters by the imidazolyl moiety of histidine containing oligopeptides.2b1 Preaently, the mechanism and origin of the observed enantioselectivities are not well understood. An understanding of the mode of adsorption of molecules a t the micellar interface and of the factors that control the interaction between these adsorbed molecules may be important for synthetic and pharmaceutical applications. In aqueous solution the imidazolyl moiety is an active catalyst in the hydrolysis of p-nitrophenyl esters. In the first step of this hydrolysis (A in Scheme I) the imidazolyl group is acylated. In the second, relatively slow step (B in Scheme I) the acetylated imidazolyl intermediate is hydrolyzed and the free imidazolyl moiety is regenerated. Upon increasing the substrate concentration typical Michaelis Menten kinetics is observed. At high substrate concentrations the catalyst is completely acylated and the (1) (a) University at Utrecht. (b) University at Nijmegen. (2) (a) Meakin, B. J. J. Pharm. Pharmocol. 1971,23,25. (b)Jhara, Y.; H d o , R.; Nango,M.; Kwoki, N. J. Chem. SOC.1985,2,5. (c) Ueoka, R.; Mwnkami, Y. Zbid. 1989,219. (d) Ihara,Y.; Kunikiyo, N.; Kunima~a, T.;Kimura, Y.; Nango, M.; Kuroki, N. Zbid. 1983,1741. (e) Ohkubo, K.; Matsumoto, N.; Nagasaki, M.; Yamaki, K.; Ogata, H. Bull. Chem. SOC. Jpn. 198457,214. (0M w , R. A.; Taguchi, T.; Bizzigotti, G.0. Tetrahedron Lett. 1982,1985. (e) Ueoka, R.; Matsumoto, Y.; Nagamatau, T.;Hirohata, S. Zbid. 1984,1363. (h) Ueoka, R.; Mataumoto, Y.; Ihara, Y. Chem. Lett. 1984, 1807. (i) Ueoka, R.; M-E, R. A.; Swamp, S.; Matsumoto, Y.; Stratus, G.; Murakami, Y. J. Am. Chem. SOC.1985,107, 2186. (j) M w , R. A.; Chiang, Y. C. P.; Hui, Y. J. Am. Chem. Soc. 1984, 106,7506. (k) Ueoka, R.; Matsumoto, Y.; Yoehino, T.;Hiroee, T.; Kikuchi, J.; Murakami, Y. Chem. Lett. 1986,127. (1) Cho, I.; Kim, G. J . Org. Chem. 1988, 53, 6189; (m) Ueoka, R.; Matsumoto, Y.; Moss, R. A.; Swamp, S.;Sugii, A.; Harada, K.; Kikuchi, J.; Murakami Y.; J. Am. Chem. SOC.1988,110,1688,

hl

I a

2

h

H-NwN' R'

O C H 2

WCH2 H

CH30

S1-L-Phe-L-HiS

Chart 11. R-Surf 16 H*C-A[

CH3 I I a

3

CH3

B@

rate is independent of the substrate concentration. This paper describes the esterolytic activity and enantioselectivity of a number of imidazole-containing dipeptide derivatives dissolved in an aqueous micellar solution. The imidazolyl moiety is part of the chiral amino acid residue L-histidine at the C-terminal end (Zposition) of the dipeptide. This C-terminal end is unprotected,

OO22-3263/91/1956-3883$O2.50/0 0 1991 American Chemical Society

Cleij et al.

3884 J. Org. Chem., Vol. 56, No. 12, 1991 Scheme I. Catalytic Cycle for the Imidazole-Catalyzed Hydrolysis of p-Nitrophenyl Esters

Table I. Rates (ka* (M-l @-I)) and Enantionelectivies ( k ~ / kof~the ) Cleavage of Clz-Phe-ONP(L and D) by Comicelles of S,*-L-X-L-Hisand R-Surf 16 at 25 O c a catalyst kLb k ~ * k ~ / k ~ S12-~-Ala-bHis 391 109 3.6 4.2 S12-~-But-~-His 537 129 141 8.3 S12-~-Norval-~-His 1171 1675 136 12.3 S12-~-Leu-~-His 3688 216 17.1 S12-~-Phe-~-His 203 17.4 S12-~-Phe-~-HisC 3531 s,,-~-Trp.~-His 251 126 2.0

0

I

HOCR veyslow

pIm

- y d o w

a Conditions: 0.08 M Tris.HC1 buffer and 0.4 M KCI; pH = 7.3; acetonitrile/water = 3/97 (v v); c dDr= 5 x IOd M c,,btnt. = 1 x 10" M;c,damt = 5 X 10- M. k k = ~ ka,obfor the L-enantiomer of the substrate and kD = kqob for the D-enantiOmer of the substrate. In the presence of S-surf 16.

/

I

A

Chart 111. Substrates

Table 11. Rates of the Cleavage of PNPA by Comicelles of S12-L-X-L-Hisand R-Surf 16' kb0b (M-' kqOb (M-' catalyst 8-1) catalyst 8-1) s,,-~-Ala-~-His 5.0 S12-~-Leu-~-His 5.8 S12-~-But-~-His 5.1 S12-~-Phe-~-His 9.0 S12-~-Norval-~-His 6.1 s,,-~-Trp-~-His 5.3 a

Abbreviations R3 = O C H 2 0

2-L or o-Phe-ONP

R3 = CHdCHzho

C I z - ~or- D-P~c-ONP

which implies that under the employed pH condition (pH = 7.3) the carboxyl moiety is deprotonated and in its anionic form. The amino acid residue at the N-terminal end is systematically varied and so is the nature of the Nprotecting group which in most cases is of the alkyloxycarbonyl (carbamate) type. All catalysts including their abbreviations are listed in Chart I. The employed surfactant is the chiral cationic surfactant (R)-N,N-dimethyl-N-hexadecyl-N-(a-methylbenzy1)ammonium bromide (R-surf 16, see Chart 11). The chiral substrates are N-protected p-nitrophenyl esters of the amino acid Lor D-phenylalanine (see Chart 111). For comparison the achiral substrate p-nitrophenyl acetate (PNPA) is also included. Attention is focused on the first step in the catalytic cycle, i.e. the acylation of the imidazolyl moiety. The enantioselectivity is expressed as the ratio of the rate constants obtained for this acylation step employing L- and Dsubstrate: k L / k D The deacylation step of the acylated imidazolyl moiety, regenerating the free imidazolyl group, is not investigated. It is our aim to understand the cause of the observed enantioselectivities.

Results Enantioselective Ester Cleavage by Histidine-Containing Dipeptides. In this section the effect is investigated of changing the nature of the amino acid residue at the N-terminal end of the L-histidine-containing dipeptide catalysts on the enantioselective hydrolysis of the long acyl chain substrates C,,-L/D-P~~-ONP. The Nprotecting group in all dipeptides is the dodecyloxycarbonyl moiety (abbreviated as SI*).The amino acid residue that is varied contains a hydrocarbon side chain of varying hydrophobicity. The only exception is tryptophane, which has an amphiphilic side chain since the NH group of the indolyl ring can form a strong hydrogen bond with water. The hydrophobicity of the amino acid side chain increases from a methyl group in the L-alanyl residue up to a benzyl moiety in the L-phenylalanyl residue.

Conditions as described in Table I.

Table I shows the results for the hydrolysis of L- and D-C12-PheONPby comicelles of S12-L-X-L-Hisand R-surf 16. The increase in hydrophobicity of the amino acid side chain of residue X from alanine up to phenylalanine is accompanied by an increase in selectivity from kL/kD = 3.6 up to 17.1. In the presence of SI2-~-Trp-~-His the selectivity is only kL/kD = 2.0. The enhancement of selectivity is almost exclusively due to the increasing rate of the L-substrate whereas the rate of the D-substrate is hardly affected. Apparently, the increase in rate of the L-substrate is due to an increased hydrophobically driven attractive interaction between catalyst and L-substrate. Such an interaction is absent with the D-substrate. The very low selectivity of the tryptophane containing catalyst is primarily due to the almost total collapse of activity toward the L-substrate. Such behavior indicates that the interaction with the substrate is not stabilized by the Trp side chain. In Table I data for the S12-~-Phe-~-His catalyst in the presence of S-surf 16 are also included. It is clearly seen that the chirality of the head group of this surfactant has no significant effect on the observed rates and enantioselectivity. The blank reactions in the absence of catalyst also display an insignificant enantioselectivity (kL/kD = 1.08 f 0.05 in the presence of R-surf 16). These observations indicate that the chiral surfactant molecules R- or S-surf 16 do not recognize the chirality of the adsorbed catalyst, substrate, or transition state. Cleavage of p-Nitrophenylacetate(PNPA)by Histidine-ContainingDipeptides. Table I1 shows the rates of cleavage of the achiral substrate p-nitrophenyl acetate (PNPA) in the presence of the micellar bound catalysts S,,-L-X-L-H~S.When Tables I and I1 are compared the most striking difference is the relatively low activity observed with PNPA. When the rates are compared with the C12-~-Phe-ONPsubstrate a 20-fold reduction is observed. This reduced activity primarily arises from the low binding affmity of the less hydrophobic PNPA ester to the micelles. At the employed surfactant concentration the vast majority of the substrate resides in the aqueous phase.3 Consequently, the rate enhancing effect of (3) Funasaki, N.J. Coll. Interf. Sci. 1978,64, 461.

J. Org. Chem., Vol. 56, No. 12, 1991 3885

Ester Cleavage by Histidine-ContainingDipeptides

(M-I d))and Enantiorelectivities Table IV. Rates ( k ~ / kof~the ) Cleavage of C12-Phe-ONP(L and D) by Comicelles of R-L-Phe-L-Hisand R-Surf 16 at 25 O C " catalyst kL kD kL/kD Z-L-Phe-L-His 1648 93 17.7 2637 149 17.7 p-BrZ-L-Phe-L-His 3067 179 17.1 F,Z-L-Phe-L-His

Table 111. Rates (kvb (M-l 8-l)) and Enantioselectivities ( k ~ / kof~the ) Cleavage of CI2-Phe-ONP(L and D) by Comicelles of S.-L-Phe-L-His and R-Surf 16 at 25 O c a

S1-L-Phe-L-Hisb Sz-L-Phe-L-Hisb SS-L-Phe-L-His S,-L-Phe-L-His Ss-L-Phe-L-His Sg-L-Phe-L-His Slo-L-Phe-L-His Slz-L-Phe-L-His S18-L-Phe-L-His

77 172 512 1705 2957 4378 5440 5983 6460

5.6 10 28 96 171 260 324 363 389

13.8 17.2 18.3 17.8 17.3 16.8 16.8 16.6 16.6

a

Table V. Rates (kW (M-l d))and Enantioselectivities ( k L / k ~of) the Cleavage of Z-Phe-ONP (L and D) by Comicelles of R-L-Phe-L-Hisand R-Surf 16 at 25 O c a catalyst kL kD kL/kD Sz-L-Phe-L-His 38.9 7.2 5.4 Z-L-Phe-L-His 297 61 4.9 694 130 5.3 F&L-Phe-L-His 1070 221 4.8 Sle-L-Phe-L-His

Conditions: 0.08 M Tris.HC1 buffer and 0.4 M KC1; pH = 7.3; acetonitrile/water = 3:97 (v/v); cmt = 5 X lod M;c,"~ = 1 X loa M;c , =~ 2.5 X M. *cat = 25 X loa M.

bringing the catalyst and substrate together in the micelles is much smaller. A clear correlation exists between the rates in Table I1 and the rates toward the Dsubstrate in Table I. They both increase to the same extent when the amino acid side chain in the catalyst becomes more hydrophobic. The rate enhancement is most pronounced for the phenylalanyl-containing catalyst whereas the rate drops for the Trp-containing catalyst. Effect of the N-Protecting Group on the Enantioselectivity. The effect of changing the hydrophobicity of the N-(alkyloxycarbonyl) protecting group of the dipeptide catalyst S,-L-Phe-L-His on the esterolytic activity and enantioselectivity toward the substrate C12-Phe-ONP (L and D) is shown in Table III. Increasing the alkyl chain length S, of the catalyst results in an enormous enhancement of the activities up to n = 10-12 after which a ceiling value is reached. The rate enhancement from S2 to SI2is about 25-30 fold. The most remarkable aspect is that, in spite of the large rate differences, the selectivities are hardly affected and remain constant around kL/kD = 16-18, except for the change from S1 to S2, i.e. it is only the part of the hydrophobic alkyl chain S, directly adjacent to the hydrophilic OC(0)NH group that affects the chiral recognition. The hydrophobic chain of the N-protecting group in the catalyst mainly functions as a hydrophobic anchor by which the catalyst is bound to the micelle. An increase in hydrophobicity of this chain will increase the fraction of catalyst that is bound to the micelles, where the very hydrophobic substrate resides, resulting in a rate enhancement. However, at SlpSls the catalyst approaches a situation in which it is completely micellar bound at the employed surfactant concentration. A further increase in hydrophobicity has no effect on the reaction rates. The data in Table I11 show that the rate becomes negligibly small when the hydrophobicity of the N-protecting group is low as in the case of S,-L-Phe-L-His. This indicates that only a very small fraction of the S1-L-Phe-L-His catalyst is bound to the micelle. If it is assumed that SlgL-Phe-L-His is completely micellar bound, this fraction can be calculated to be no more than 1-2%. This result is remarkable since the S,-L-Phe-L-Hiscatalyst still contains the very hydrophobic side chain of the phenylalanyl residue. Apparently, this side chain, which is located between two hydrophilic moieties, cannot dissolve into the micellar hydrocarbon phase and contribute to the binding strength of the catalyst to the micelle. Table IV shows rate data for N-(benzyloxycarbonyl)(Z) and substituted N-(benzyloxycarbonyl)-protected The observed selectivities, k L / k D = 17-18, indicate that the mode of interaction of these catalysts with the micelle and with the C12-Phe-ONP(L and D) substrates is identical to that of the N-(alkyloxycarbonyl) protected catalysts.

Conditions as described in Table 111.

a

Conditions as described in Table 111.

Table VI. Rates (k.,+ (M-l d))and Enantioselectivities ( k L / k ~of) the Cleavage of 2-Phe-ONP and Cl,-Phe-ONP (L and D) by Comicelles of His-Containing Dipeptides and R-Surf 16 at 25 O c a ~

~~~

Cle-Phe-ONP Z-Phe-ONP kL k~ k ~ / k ~&L kD kL/kD

catalyst S1,-D-Phe-L-His 1889 362 Clz-L-Phe-L-His 1451 251 16 3 C,-L-Phe-L-Hisb 358 89 Z-L-Ala-L-His a

3.0 5.8 5 4.0

478 218 378 225 3.2 1.4 149 59

2.2 1.7 2.3 2.5

Conditions as described in Table 3. * c, = 5 X lo-' M.

The activity of Z-L-Phe-L-His corresonds to the activity of S,-L-Phe-L-His (Table 111),indicating that the hydrophobicity of a Z moiety is identical with the hydrophobicity of an S4 moiety. This would mean that a phenyl and a n-propyl group have equal hydrophobicities. This conclusion is in agreement with the almost equal free energies of transfer of benzene and propane from water to a liquid hydrocarbon at 25 "C. These energies amount to -4.6 and -4.9 kcal/mol, respectively? It is also in agreement with the identical free energy changes for transfer of the amino acids phenylalanine (benzyl side chain) and norleucine (n-butyl side chain) from water to an organic solvent? The higher activities observed for the p-BrZ- and F5Zprotected catalysts are in line with the fact that these moieties are more hydrophobic than the unsubstituted Z moiety. The activity of the F$ moiety in comparison with the Z moiety corresponds to an increased hydrophobicity of two methylene groups in an unbranched hydrocarbon chain. The substitution of the para hydrogen by a bromine atom corresponds to an increased hydrophobicity of approximately 1.7 CH2 groups. Table V presents the activity and enantioseletivity of comicelles composed of R-L-Phe-L-Hisand R-surf 16 towards the chiral substrates Z-Phe-ONP (L and D). Again, the enantioselectivities are not significantly affected by the degree of hydrophobicity of the N-protecting group in the catalysts. The rate enhancement is approximately 2530-fold when the hydrophobicity of the N-protecting group increases from S2 to S12.This rate enhancement is identical with the one observed for the long acyl chain substrates C12-Phe-ONP. The selectivities, however, are markedly lower, suggesting a less favorable fit of the former substrates and the catalyst in the transition state. The (4)Mc Auliffe,C. J.>hys. Chem. 1966,70, 1267. (5) (a) Nozaki, Y.;Tanford, C. J. Biol. Chem. 1971,246, 2211. jb) Tanford, C.The hydrophobic effect: formotion of micelles and biobgzcal membranes, 2nd ed.; Wiley-Interscience: New York, 1980; p 23.

3886 J. Org. Chem., Vol.56,No.12, 1991

reduced selectivities in comparison with the C12-Phe-ONP substrates are mainly due to a reduced activity toward the L-substrate. In Table VI the activities and enantioselectivities of some additional L-histidine-containing catalysts toward the substrates C12-Phe-ONPand Z-Phe-ONP are given. The activities obtained for S12-o-Phe-L-His(entry 1)should be compared with those of the diastereomeric catalyst SI2L-Phe-L-His in Tables I11 and V. The enantioselectivity appears to depend strongly on the configuration of the phenylalanyl residue in the catalyst. The selectivityk L / k D = 17 toward C12-Phe-ONPobserved with the L-Phe-L-His catalyst is reduced to only kL/kd = 3 with the o-Phe-L-His catalyst. The reduction in selectivity is exclusively due to a 5-6-fold decrease in activity towards the L-substrate. The activity toward the D-substrate is not affected to a significant extent. A very similar, although smaller, effect is observed for the Z-Phe-ONP substrate. These results again demonstrate the intimate involvement of the Phe residue of the catalyst in the chiral recognition of the substrate. Entry 2 of Table VI shows the results of the esterolysis of C12-Phe-ONPby Clz-L-Phe-L-His. The data should be compared with those for the S12-~-Phe-~-His catalyst in Table 111. The difference between the two catalysts is that the former is protected with a dodecanoyl group and the latter with a dodecyloxycarbonyl group. Both protecting groups have similar hydrophobic parts. The C12-~-PheL-His catalyst exhibits a much lower selectivity ( k L / k D = 5.8) than the Slz-L-Phe-L-Hiscatalyst (kL/kD = 17). This reduction in selectivity is mainly due to a 4-fold decrease in reaction rate of the L-substrate, whereas the rate of the D-substrate is only slightly affected. This suggests that the carbamate moiety in the S12-protectedcatalyst is involved in the interaction of the catalyst with the L-substrate in the transition state. Replacing the carbamate moiety by an amide group apparently reduces this interaction. Note that in the previous section it was observed that the opposite occurs for the substrate, i.e. with the C12-protectedsubstrate (amide) higher enantioselectivities and activities are obtained than with the Z-protected substrate (carbamate). Entry 3 of Table VI gives the results obtained with the N-acetyl-L-Phe-L-His catalyst. Both the activities and enantioselectivitiesare very low. The activity is even lower than that of S1-L-Phe-L-His(Table In), indicating that the interaction of the catalyst with the micelles is very weak. Most of the catalyst will reside in the aqueous phase. If the activities of C1-L-Phe-L-Hisand C1+-Phe-L-His (Table VI, entries 2 and 3) toward the substrate C12-Phe-ONPare compared, it can be concluded that no more than 1% of the former catalyst is bound to the micelles. Entry 4 of Table VI shows the activity and enantioselectivity of Z-L-Ala-L-His toward the esters C12-Phe-ONP and Z-Phe-ONP. The enantioselectivity toward C12-PheONP ( k L / k D = 4.0) is nearly identical with the one observed with the much more hydrophobic catalyst S12+ Ala-L-His (Table I, k L / k D = 3.6) only the rates are reduced due to the lower binding to the micelles. A similar behavior was observed for the catalysts Z-L-Phe-L-His and s,,-~-Phe-~-His (Tables IV and 111). It is of interest to compare the activities of the Z-L-Ala-L-His and the S1-LPhe-L-His catalysts (Tables VI and 111). On the basis of the structural formula both catalysts can be classified as equally hydrophobic. The methyl and benzyl moiety have changed their positions in these catalysts. However, the catalytic activity of Z-L-Ala-L-His is much higher (up to 15-fold for the D-substrate), indicating that a much larger

Cleij et al. Table VII. Rates (k,b (M-l d)) and Enantioselectivitier ( k L / k Dof) the Cleavage of C12-Phe-ONPby Comiceller of Slt-L-Phe-L-Hisand R-Surf 16 at Various Temperatures" T ("C) kL kD k ~k~l 5 15 25 35 45 50 a

456 185 1106 1217 1229 1249

15 32 63 113 181 218

30.4 24.5 17.6 10.8 6.8 5.7

Conditions as described in Table I; c,& = lo-* M.

''-

6.0

J ?

U 0.0032 0.0034 0.0036 1/T (k")

B 2

4

\ 0.0032 0.0034 0.0036 1IT (IC")

Figure 1. (a) In KL as a function of 1/T. (b)In k~ as a function of 1/T (data from Table VII).

fraction of this catalyst is bound to the micelles. The benzyl moiety in Z-L-Ala-L-His is not located between two hydrophilic groups and can efficiently interact with (dissolve into) the hydrocarbon phase of the micelles. Effect of Temperature. The effect of the temperature on the catalytic activity of S12-L-Phe-L-Histoward ClzPhe-ONP in the presence of R-surf 16 is shown in Table VII. A relatively high surfactant concentration is chosen M) in order to be sure that both catalyst and substrate remain completely bound to the micelles over the entire temperature range. Above 25 OC, the activity toward the L-substrate is severely suppressed, i.e. the activity remains almost constant although the temperature is raised. Similar behavior is observed for enzymes that often display a maximum activity at a certain temperature. This phenomenon is not observed for the catalytic activity toward the D-substrate which increases regularly above 25 "C.In Figure 1,parts a and b, In k is plotted against 1/T. With the D-substratean almost linear plot is obtained, but with the L-substrate a strong deviation from linearity above 25 OC is observed. It is clear that this behaviour will strongly reduce the enantioselectivity (see Table VII). These results indicate that upon raising the temperature a favorable interaction that exists between the catalyst and the L-substrate, is severely reduced. Such an interaction does not exist with the D-substrate. Fluorescence Measurements on the TryptophaneContaining Catalyst. The position of the fluorescence spectrum of Trp strongly depends on the polarity of the microenvironment. The emission spectrum of Trp-containing probes in a solution of micelles not only furnishes information about the average polar surroundings of micellar bound molecules but also gives information about the heterogeneity or distribution of the probe between the aqueous and micellar

Ester Cleavage by Histidine-Containing Dipeptides

J. Org. Chem., Vol. 56,No. 12, 1991 3887 a

Table VIII. Fluorescence Maximum of S,+TrpL-His Dissolved in Dioxane-Water Mixturesa solvent mixtureb E ~ ( 3 0 )(kcal/mol)' AF (dd 0 63.1 360 10 20

61.1 58.7 57.1 65.5 53.9 52.3 50.7 49.1 46.8 36.1

30 40 50 60 70

80 90 100

359 357 354 352 351 349 348 346 343 333

Water

L3

Micelle b

.cl

T = 25 "C;cPmb = 2 X 10" M. bVolume percentage dioxane in water. 'Values taken from ref 17 or from data in this reference by linear interpolation. Wavelength of maximum fluorescence intensity ( a 1 nm) at an excitation wavelength of 286 nm. a

11.1

C

0

1

2 3 4 conc. R-surf 16 I mM

5

Figure 2. The ositions of the fluorescence emission maximum of SIT~-Trp-~& in a surfactant solution of R-surf 16. X, = 286 nm;0.08 M Tris.HC1; 0.40 M KC1; pH = 7.3;cPmb= 2 X lob M.

The probe SI2-L-Trp-L-Hiswas added to a solution of R-surf 16 under reaction conditions. Subsequently, a fluorescence spectrum was recorded. For comparison, the fluorescence emission spectrum of the Trp-containing catalyst was also measured in various 1,4-dioxane-water mixtures. The position of the emission maximum in these mixtures is presented in Table VIII, together with the corresponding solvent polarities expressed by the ET(30) parameter.& Upon increasing the surfactant concentration the emission maximum of the catalyst gradually shifts from 360 nm (surfactant free buffer solution) to 351 nm (completely micellar bound catalyst at approximately 2 mM, Figure 2). The emission maximum of the completely micellar bound catalyst corresponds to a polarity of 54 ) or to a 50%/50% (v/v) kcal/mol on the E ~ ( 3 0scale 1,4dioxanewater mixture. This clearly indicates that the indolyl moiety is not completely dehydrated but remains exposed to the aqueous phase.

Discussion If amphiphilic molecules like our catalysta and substrates are added to an aqueous micellar solution, the apolar hydrocarbon parts of these molecules will dissolve into the micellar hydrocarbon phase, whereas the polar hydrophilic parts will tend to remain in the aqueous phase. However, the hydrophobic groups in the catalyst or substrate that are in close proximity to hydrophilic groups will not be able to dissolve into the micellar hydrocarbon phase without causing dehydration of these hydrophilic groups, (6). (a) Lakowicks,J. R.J. Biol. Chem. 1983,258,5619. (b) Permyakov, M. Bzophys. Chem. 19sS,18, 145. (c) Irace, G. Biochemistry 1981,20, 792. (d) Shinitzky, M. Biochemistry 1977,16,982. (e) The intramolecular charge-transfer process of Trp can be best compared with a solvent polarity parameter based on a similar Intramolecular charge-transfer proms, e.g. the E ~ ( 3 0parameter. ) For a diecussion see: Kmwer, E. M.; Dodiuk, H.; Kanety, H. J. Am. Chem. SOC.1978,100, 4179.

Figure 3. (a) The formation of a hydrogen bond at the micellar interface between the catalyst and the L-enantiomer of the substrate. (b) Schematic representation of the tetrahedral intermediate 1 that is formed from the s,-L-Phe-L-His catalyst and the CI2-L-Phe-ONPester. The hydrophobic parta of the N-protecting groups are not shown. The hydrogen bonds between the L-Phe and L-His residue (C,) and between both L-Phe residues are represented by dotted lines. (c) A CPK space-filling model of 1.

i.e., they must remain in the aqueous phase. The apolar amino acid side chain of the amino acid residue X adjacent to the His residue in the catalyst and the amino acid side chain of the substrate, which are both located between two hydrophilic groups, will remain exposed to the aqueous phase when these molecules are adsorbed to the micellar interface (Figure 3a). Also the CH2 groups of the hydrophobic alkyl chain of S, in the catalyst that are adjacent to the hydrophilic OC(0)NH group will remain exposed to the aqueous phase, the rest of this alkyl chain is free to dissolve into the micellar hydrocarbon phase. The hydrophilic-hydrophobic conflict can be solved in the following way: if the polar hydrated groups form hydrogen bonds with each other, they lose their hydrophilicity and are free to dissolve in an apolar environment which allows the transfer of the adjacent hydrophobic groups to the apolar micellar phase (Figure 3a). When dipeptides are dissolved in apolar solvents, they This conformation adopt the so-called C, is characterized by an intramolecular hydrogen bond be(7! (a) Ramachandran,J. Mol. Biol. 1963, 7, 95. (b) Bricas, E., Ed. Peptides 1968; North-HollandPublishing Company: Amsterdam,1968. (c) Walbn, A. G. Polypeptides and Protein Structure; Elsevier: New York, 1981. (d) Udenfriend, S.; Meienhofer, J. The Peptides, Analysis, Synthesis, Biology; Academic Press Inc.: New York, 1985; p 84.

Cleij et al.

3888 J. Org. Chem., Vol. 56, No.12,1991

tween the adjacent amide groups. A seven-membered ring is formed. If our S,-L-Phe-L-His catalyst attains the C, conformation, one side of the amino acid side chain of Phe can adsorb to the micellar hydrocarbon interface. The CO moiety of the N-protecting group and the NH moiety of the His residue form the intramolecular hydrogen bond, and the NH and CO moieties of the Phe residue remain hydrated. In this position the amino acid side chain of the Phe residue lies flat on the micellar interface, and the alkyl chain of the N-protecting group points to the center of the micelle. Figure 3, parts b and c, gives a top view on the micellar interface of the tetrahedral intermediate 1 that is proposed for the reaction between the S,-L-Phe-L-His catalyst and the CI2-~-Phe-ONP substrate. This intermediate closely resembles the transition state. The NH group of the Phe residue of the catalyst forms an intermolecular hydrogen bond with the amide CO group of the L-substrate. This allows the adjacent apolar groups to be dissolved in the micellar hydrocarbon phase. The larger these apolar groups are (from X = Ala to X = Phe, and from S1to S,) the more stable this transition state will be. In 1, the p-nitrophenyl moiety is adsorbed to the micellar interface. The proposed conformation is (4,J/,x',x2) hs,estalyet = -looo, TO0, g,No; (4,x2,x2)m= -120°, K, 90'; hx1,x2)pheaUbhk = -looo,g,90' (4 is the torsional angle around the N-Ca bond, J/ around the C W O bond, x1 around CWY, and x2 around C5-C7).'3 These are all low energy conformations. N-Acetyl-~-Phe-N-methylamide~JO can be considered as the structural element of the Phe residue in the S,-LPhe-L-His catalysts and the L-substrates. In the crystalline state this molecule has the conformation 4,x1,x2= - 1 0 6 . 7 O , g,89.8O. This is essentially identical with the conformation in the proposed transition state 1. In addition a hydrogen bond is present between the molecules that is similar to the proposed hydrogen bond in 1. Model building shows that the D-enantiomer of the substrate cannot form a tetrahedral intermediate with an L,L-catalyst,in which an intermolecular hydrogen bond is formed that allows the transfer of all hydrophobic groups to the micellar hydrocarbon phase. If the Phe residue of the catalyst is changed from L into D, the interaction of the D-substratewith the DPhe residue in the D,L-catalyst can be identical with and just as favorable as the interaction between the L-substrate and SI2-~-Phe-~-His, shown in 1. The kinetic data, however, show that in comparison to the L,ccatalyst the D , L - c a d p t exhibits no enhanced activity toward the D-substrate. Model building shows that the imidazolyl moiety cannot reach the ester group. The side chain of the Trp residue is amphiphilic. Consequently,it is not favorable to transfer this side chain to the micellar hydrocarbon phase when 1 is formed, unless the L-substrate can form a hydrogen bond with the NH part of the indolyl moiety. Since this is not the case, the transition state will not be stabilized. The kinetic data in Table I for SI2-~-Trp-~-His show that the rate toward the L-substrate even falls below the rate observed with the Ala-containing catalyst. Steric Effects. Upon formation of the tetrahedral intermediate 1, the N-protecting groups of the catalyst and (8)The nomenclature and conventions used follow the recommendations of the IUPAC-IUB Commission on Biochemical Nomenclature 8% Biochemistry 1970, 9, 3471. (9) (a) Hmadat y.BiochemktO' 1977, B% 244. (b)ICkhWa, T. m i . 1977, B25,1824. (10) Harada, Y. Acta Crystollogr. 1974, B90, 726. (11) Benedetti, E.; Pedone, C.; Toniolo, C.; Dudek, M.;Nemethy, G.; Scheraga, H. A. Znt. J. Pept. Protein Res. 1983,21, 163.

aqueous phasc

IMG'= 1.7 kcal /moll

IAA+=

0.9 kcal /mol

1

aqueous phase

----.---..--.--.......--..-*-.--.----.----.....-.interface

Figure 4. Steric effects of the N-protecting groups in 1. substrate approach each other very closely. The hydrophobic parts of these N-protecting groups, which are dissolved in the micellar hydrocarbon phase should preferentially point away from each other. This is the case when the catalyst is N-protected with an alkyloxycarbonyl moiety (S,-L-Phe-L-His; see Figure 4a which shows the low energy 2 conformationlo)and the L-substrate with an acyl moiety (CI2-~-Phe-ONP; see Figure 4a). If the substrate is N-protected with an alkyloxycarbonyl moiety or the catalyst with an acyl moiety, the formation of the hydrogen bond and thus the transition state with the L-substrate is hindered (Figure 4, parts b and c, respectively). When the catalyst is protected with an acyl moiety and the L-substrate with an alkyloxycarbonyl moiety, the steric hindrance is the largest (Figure 4d). The experimental data show that the reduced enantioselectivities are almost exclusively due to a reduced activity toward the L-substrate, Le. only the formation of the transition state with the L-substrate is suppressed. Conclusions From the data presented in this paper the following conclusions can be drawn. (1)The amphiphilic catalysts and substrates are adsorbed to and oriented at the micellar interface. (2) Not all the hydrophobic parts of the catalyt and the substrate can dissolve completely into the micellar hydrocarbon phase due to the need for hydration of the hydrophilic groups. (3) Of the two diastereomeric transition states, only the transition state with the L-enantiomer of the ester has a hydrogen bond between the ester and the catalyst. (4) The hydrogen bonded groups lose their hydrophilicity, which allows the transfer of these groups and the adjacent hydrophobic moieties to the micellar hydrocarbon phase. This stabilizes the transition state. (5) Steric hinderance between the N-protecting groups of the catalyst and the L-substrate opposes the formation of this stabilizing hydrogen bond. In the present case, the least steric hinderance occurs when the catalyst is protected by an alkyloxycarbonyl group and the substrate by an acyl group. Experimental Section General Remarks. Thin layer chromatography (TLC) was performed on (Mer& DC-Plastikrolle, Kieselgel 60 Fm), and detection was effected by ultraviolet light or iodine. Column chromatography was performed with silica (Merck Kieselgel60, 23&400 mesh). Solvents and reagents were of analytical grade.

Ester Cleavage by Histidine-Containing Dipeptides Synthesis. (Alkyloxycarbony1)-L-(or D)-Amino Acids (S,-L-(or D)-X-OH), (Benzyloxycarbonyl)-L-PheOH,(Benzyloxycarbony1)-L-Ala-OH, (2,3,4,5,6-Pentafluorobenzyloxycarbonyl)-L-Phe-OH, ( p-Bromobenzyloxycarbonyl)-LPhe-OH. These compounds were prepared by coupling of the chloroformates with the corresponding amino acids according to a literature method.12 The yields amounted to 60-70%. The IR spectra (NaC1, KBr, or neat) of all compounds showed bands at 3300 (NH carbamate), 1720 (COOH), 1685 cm-' (C=O carbamate), unless noted otherwise. TLC: R = 0.3-0.4 (chloroform-methanol, 4/1, v/v) for all compounds. The compounds had the following physical properties: 'H NMR (CDClJ; [(r]"OD (c = 1.0, methanol) unless noted otherwise; mp, 'C. S12-~-Ala-OH:6 0.9 (t,3 H, CHJ, 1.3 (m, 20 H, (CH2),0), 1.45 (d, 3 H, CHJ, 4.05 (t, 2 H, CHZO), 4.3 (2 9, 1H, CH), 5.5 (d, 1 H, NH), 10.9 ( 8 , 1 H, COOH) ppm; -12.7'; 68.8. S12-~-But-OH (from a-aminobutyric acid): 6 0.9 (t,3 H, CH3), 1.0 (t, 3 H, CHCH2CH3),1.3 (m, 20 H, (CHz)lo),1.65 (m, 2 H, CHCHZCHJ, 4.0 (t, 2 H, CHZO), 4.25 (2 t, 1H, CH), 5.4 (d, 1H, NH), 10.5 ( 8 , 1 H, COOH) ppm; -10.8'; 70.5. S12-~-Norval-OH:6 0.9 (t,6 H, 2 CH3),1.3 (m, 24 H, (CHJlo and CHCH2CHzCH3),4.0 (t, 2 H, CHZO), 4.2 (2 t, 1 H, CH), 5.1 (d, 1 H, NH), 10.4 (8, 1 H, COOH) ppm; -9.8'; 55.4. Slz-L-Leu-OH: 6 0.9 (t, 3 H, (CH,),O-CH,), 0.9 (2 d, 6 H, CH(CH3)2),1.3 (m, 23 H, (CH2)10and CH2CH(CH3)2),4.0 (t, 2 H, CH20), 4.05 (2 t, 1 H, CH), 5.4 (d, 1 H, NH), 10.7 (8, 1 H, COOHj ppm; -8.1'; oil. S12-L-Phe-OH: 6 0.9 (t, 3 H, CH3),1.3 (m, 20 H, (CH2)lo,3.15 (d (dist), 2 H, CHzPh);4.0 (t,2 H, CH,), 4.65 (2 t, 1H, CH), 5.2 (d, 1 H, NH), 7.2 (8, 5 H, ArH), 11.4 (s (br), 1H, COOH) ppm; -2.8', oil. Slz-L-Trp-OH: 6 0.9 (t, 3 H, CH3),1.3 (m, 20 H, (CH2)3,3.25 (d (dist), 2 H, CH2-indolyl),4.0 (t, 2 H, CH20),4.6 (2 t, 1 H, CH); 5.25 (d, 1 H, NH), 6.7-7.7 (m, 5 H, indolyl), 8.1 (a (br), 1 H, NH (indolyl)), 8.8 (s (br), 1 H, COOH) ppm; -3.2'; 123.2. Z-L-Phe-OH: 6 3.05 (d (dist), 2 H, CHCH2Ph),4.45 (2 t (dist), 1 H, CH), 4.9 ( 8 , 2 H, CHzO),5.45 (d, 1H, NH), 7.1 and 7.15 (2 s, 2 X 5 H, 2 Ph), 11.0 (s, 1 H, COOH) ppm; +5.1' (c = 1.0, glacial acetic acid); 88.1. p-BrZ-L-Phe-OH: 6 3.1 (d (dist), 2 H, CHCH2Ph),4.5 (2 t (dist), 1H, CH), 5.0 (8, 2 H, CH,O), 5.3 (d, 1 H, NH), 7.1 (8, 5 H, C&), 6.9 and 7.3 (s d, 2 X 2 H, C6H4Br),10.1 (s (br), 1H, COOH) ppm; -9.2'; 108.7. F&L-Phe-OH: 6 3.3 (d (dist), 2 H, CH2),4.6 (2 t (dist), 1H, CH), 5.1 (9, 2 H, CH2), 5.2 (d, 1H, NH), 7.2 (m, 5 H, Ph), 9.45 (9, 1 H, COOH) ppm; -9.4'; 134.8; IR (KBr) 1705 (w) and 1660 cm-l ( 8 ) (C=O carbamate). 2-L-Ala-OH: 6 1.45 (d, 3 H, CH,), 4.3 (2 q (dist), 1 H, CH), 4.9 ( 8 , 2 H, CHZO), 5.2 (d, 1H, NH), 7.1 (8, 5 H, Ph), 10.5 ( 8 , 1 H, COOH) ppm; -14.2'; 83.2. S1-L-Phe-OH: 6 3.15 (d (dist), 2 H, CHz), 3.6 (8, 3 H, CH3), 4.5 (2 t, 1 H, CH), 5.2 (d, 1 H, NH), 7.2 (8, 5 H, Ph), 10.4 (s, 1 H, COOH) ppm; -4.7'; oil. S2-L-Phe-OH: 6 1.15 (t,3 H, CHJ, 3.0 (d (dist), 2 H, CH,Ph), 4.0 (4, 2 H, CHz), 4.5 (2 t, 1 H, CH), 5.3 (d, 1 H, NH), 7.2 (9, 5 H, Ph), 10.2 (s (br), 1 H, COOH)ppm; -4.0'; oil. The 'H NMR and IR spectra of s3,s&,S&s10' and S16-~-Phe-OH (all viscous oils) are all very similar to the spectrum of the S12-~-Phe-OH compound. [.]"OD: -3.8', -3.5', -3.4', -3.2', -3.0', and -2.5', respectively. L-Histidine Methyl Ester Dihydrochloride. This compound was a commercial product from Aldrich. (Alkyloxycarbony1)-L-X-L-histidine Methyl Ester (S,-LX-L-His-OMe), (Benzyloxycarbonyl)-L-phenylalany1-Lhistidine Methyl Ester (Z-L-Phe-L-His-OMe), (2,3,4,5,6pentafluorobenzyloxycarbonyl)-L-phenylalanyl-L-histidine

Methyl E s t e r (F,Z-L-Phe-L-His-OMe), (Benzyloxycarbonyl)-L-alanyl-L-histidineMethyl Ester (2-L-Ala+ Hio-OMe), ( p -Bromobenzylosycarbonyl)-L-phenylalanylL-histidine Methyl Ester (p-BrZ-L-PheL-His-OMe). Coupling of the oxycarbonyl-protected amino acids with the methyl ester of thistidine was accomplished using 1,6-dicyclohexylcarbodiide (12) (a) Bergman, M.; Zervae, L. Chem. Ber. 1932, 65, 1192. (b) Farthing, A. C. J. Chem. SOC.1960,3213, (c) Houben Werl Methoden

der orginischen Chemie, 1511 (4th ed.), pp 47-80.

J. Org. Chem., Vol. 56,No. 12, 1991 3889 according to a method described in 1iterat~re.l~The crude products were purified by column chromatography (Silica 60, chloroform-methanol, 20/1, v/v) and recrystallization from ethyl acetateheme. The yields amounted to 60-70%. IR (KBr): 3300 (NH amide and carbamate), 1732 (C=O ester), 1695 (c=o amide), unlw noted otherwise. TLC carbamate), 1645 cm-l (c-0 (Silica): Rf = 0.4 (chloroform-methanol, 4/1, v/v) for all compounds. 'H NMR (CDCl,); [a]"D (c = 1.0, methanol); mp 'c. S12-~-Ala-~-His-OMe: 6 0.9 (t, 3 H, CH3), 1.3 (m, 20 H, (CHz)lo),1.45 (d, 3 H, CH3),3.15 (d (dist), 2 H, CHz-Im),3.7 (8, 3 H, OCH3),4.0 (t, 2 H, CHzO),4.2 (2 q, 1H, CH (Ala)), 4.75 (2 t (dist), 1H, CH (His)5.7 , (d, 1H, NH (carbamate)),6.7 and 7.45 (2 s, 2 x 1H, 2 CH (Im)), 7.55 (d, 1H, NH (amide)), 10.1 (8, br), 1 H, NH (Im)) ppm; -9.OO; 118.6. S12-~-But-~-His-OMe; 6 0.9 (t, 3 H, (CH2)loCH3),1.0 (t, 3 H, CHJ, 1.3 (m, 22 H, (CH2)loand CHCH2CH3),3.1 (d (diet), 2 H, CH2(His)), 3.65 (s,3 H, OCH3),4.0 (t, 2 H, CH20),4.1 (2 t (dist), 1 H, CH (But)), 4.8 (2 t (dist), 1H, CH (His)), 5.7 (d, 1 H, NH (carbamate)), 6.7 and 7.45 (2 s, 2 x 1H, 2 CH (Im)), 7.8 (d, 1H, NH (amide)), 9.2 (s (br), 1 H, NH (Im)) ppm; -9.5'; 107.8. S12-~-Norval-~-His-OMe: 6 0.9 (2 t, 2 X 3 H, 2 CHJ, 1.3 (m, , (8, 24 H, (CH2)loand (CH2),), 3.1 (d (dist), 2 H, CHz (His))3.65 3 H, OCH3),4.0 (t,2 H, CH,O), 4.15 (2 t (dist), 1H, CH (Nowal), 4.8 (2 t, 1 H, CH (His)), 5.8 (d, 1H, NH (carbamate)), 6.7 and 7.45 (2 s, 2 x 1H, 2 CH (Im)), 7.7 (d, 1 H, NH (amide)), 9.5 (8, br), 1H, NH (Im)) ppm; -9.4'; 110.9. S12-~-Leu-~-His-OMe: 6 0.9 (m, 9 H, 3 CH3), 1.25 (m, 23 H, (CHJlo and CHzCH (Leu)), 3.1 (d, 2 H, CH2 (His)),3.65 (s,3 H, OCH3),4.0 (t, 2 H, CHzO),4.15 (2 t (dist), 1 H, CH (Leu)), 4.8 (2 t, 1H, CH (His)) 5.5 , (d, 1H, NH (carbamate)), 6.7 and 7.45 (2 s, 2 x 1 H, 2 CH (Im)), 7.45 (d, 1H, NH (amide)), 8.9 (s (br), 1H, NH (Im)) ppm; -16.8'; 104.8. S,,-L-Phe-L-His-OMe: 6 0.9 (t, 3 H, CH3), 1.3 (m, 20 H, (CH2)10),3.1 (2 d (dist), 2 X 2 H, CHz(Phe)and CHz(His)),3.65 (s,3 H, OCHJ, 3.95 (t, 2 H, CH20),4.3-5.1 (m, 2 X 1H, CH (Phe) and CH (His)), 6.7 and 7.45 (2 s, 2 X 1H, 2 CH (Im)), 7.2 (8, 5 H, Ph), 7.55 (d, 1H, NH (amide)),8.9 (s (br), 1H, NH (Im))ppm; -7.4'; 118.2. SlrDPheL-His-OMe: the 'H NMR spectrum is identical with the spectrum of the Slz+Phe-L-His-OMe diastereomer; +l.Oo; 121.3. SIZ+Trp+His-OMe: 6 0.95 (t, 3 H, CHd, 1.3 (m, 20 H, (CHz)lo),3.1 (m, 2 X 2 H, CHz (Trp) and CHz (His)),3.6 (s,3 H, OCH3),4.0 (t, 2 H, CH20),4.6 (m, 2 H, CH (Trp)and CH (His)), 5.65 (d, 1H, NH (carbamate)), 6.55 and 7.35 (2 s, 2 X 1H, 2 CH (Im)),6.8-7.7 (m, 5 H, 5 CH (indolyl)),7.55 (d, 1H, NH (amide)), 8.7 (s (br), 1H, NH (Im)), 8.95 (s (br), 1H, NH (indolyl)) ppm; -7.9'; 113.5. Z-L-PheL-His-OMe:6 2.4-3.3 (m, 2 X 2 H, CH2(Phe) and CH2 (His))3.55 , (8, 3 H, OCH,), 4.3-5.0 (m, 2 X 1 H, CH (Phe) and CH (His)), 5.05 (8, 2 H, CH2 (Z)), 6.7 and 7.55 (2 s, 2 X 1 H, 2 CH (Im)), 5.6 (d, 1 H, NH (carbamate)), 7.0 and 7.25 (2 s, 2 X 5 H, 2 Ph), 7.7 (d, 1H, NH (amide)), 8.9 (s (br), 1H, NH (Im)) ppm; -8.8'; 101.3. F,Z-L-Phe-L-His-OMe (methanol-d~/DMSO-d6):6 2.7-3.3 (2 d (dist), 2 X 2 H, CHz (Phe) and CH2 (His)), 3.55 (s,3 H, OCHJ, 4.0-4.5 (2 t (dist), 2 X 1 H, CH (Phe) and CH (His)), 5.05 (8, 2 H, CHz (Z)), 7.18 (s,5 H, Ph), 7.1 and 8.2 (2 s, 2 X 1H, 2 CH (Im)) ppm; -14.9'; 151.5; IR (KBr) 1709 cm-' ((2-0 carbamate). p-BrZ-L-Phe-L-His-OMe: 6 2.4-3.3 (m, 2 X 2 H, CH2 (Phe) and CH2 (His)),3.6 (s,3 H, OCH3),4.3-5.0 (m, 2 X 1H, CH (Phe) and CH (His)), 5.1 (8, 2 H, CHzO), 6.7 and 7.6 (2 s, 2 X 1 H, 2 CH (Im)), 5.5 (d, 1H, NH (carbamate)), 7.1 ( 8 , 5 H, C&), 7.0 and 7.4 (2 d, 2 X 2 H, C6H4Br),7.8 (d, 1H, NH (amide)), 9.1 (8, 1 H, NH (Im)) ppm; -12.7'; 128.0. Z-L-Ala-L-His-OMe: 6 1.4 (d, 3 H, CH,), 3.1 (d (dist), 2 H, , ( 8 , 3 H, OCH3),4.25 (2 q, 1 H, CH (Ala)), 4.8 (2 CH, (His))3.7 t, 1 H, CH (His)), 5.7 (d, 1 H, NH (carbamate)), 6.6 and 7.35 (2 s, 2 X 1H, 2 CH (Im)),7.7 (d, 1H, NH (amide), 9.7 (s (br), 1H, NH (Im)) ppm; -10.4'; 114.2. S,-L-PheL-His-OMe: 6 3.05 (m, 2 X 2 H, CH2(Phe) and CHZ (His))3.4 . (s. 3 H. CH, (SI)). 3.6 (9, 3 H, OCHA 4.4-5.1 (m, 2 X 1H,'CH (Phe) and CH (Hh)), 5.7 (d, 1H, NH !carbamate)), 6.65 (13) (a) Houben Weyl Methoden der Organischen Chemie, 15/2 (4th ed), pp 103-113. (b) Wunsch, E. Chem. Ber. 1967, 100, 173.

3890 J. Org. Chem., Vol. 56, No. 12, 1991

Cleij et al.

p-BrZ-L-Phe-L-His-OH. 6 3.1 (2 d (dist), 2 X 2 H, CH2(Phe) and CH2 (His)), 4.1-4.6 (m, 2 x 1H, 2 CHI, 5.0 (s,2 H, CH,O), 7.2 (8, 5 H, C6H6),7.2 and 8.4 (2 8, 2 X 1 H, 2 CH (Im)), 7.0 and 7.3 (2 d, 2 X 2 H, C6H4Br)ppm; +14.9'; 191.6. Anal. Calcd for CzsHzsN40sBr:C, 53.59; H, 4.50; N, 10.87; 0, 15.52; Br, 15.52. Found: C, 53.71; H, 4.52; N, 10.99; 0, 15.49; Br, 15.62. Z-LA~~-L-H~S-OH 6 1.45 (d, 3 H, CHS), 3.1 (d (dist), 2 H, CH2 (His)), 4.3 (t, 1 H, CH (Ala)), 4.5 (t, 1H, CH (His)),4.95 (s,2 H, CH20),7.2and 8.4 (2 s,2 X 1 H , 2 CH (Im)),7.2 (s,5 H,Ph) ppm; +14.8'; 198.7. Anal. Calcd for Cl,Hd4O6 C, 56.67; H, 5.59; N, 15.55; 0,22.20. Found: C, 56.72; H, 5.59; N, 15.58; 0,22.12. S1-L-Phe-L-His-OH: 6 3.0 (m, 2 X 2 H, CH2 (Phe) and CH2 (His)),3.5 (8, 3 H, CH30), 4.0-4.7 (2 t (dist), 2 x 1H, CH (Phe) 7.2 (s,5 H, and CH (His)),7.2 and 8.4 (2 8.2 X 1H, 2 CH (Im)), Ph) ppm; +20.1°; 100.7. Anal. Calcd for C1,H&J406 C, 56.67; H, 5.59; N, 15.55; 0, 22.20. Found C, 56.74; H, 5.62; N, 15.45; (2,3,4,5,6-Pentafluorobenzyloxycarbonyl)-~-phenylalanyl- 0, 22.20. S2-~-Phe-~-His-OH: 6 1.15 (t, 3 H, CHS),2.7-3.3 (m, 2 X 2 L-histidine, (p-Bromobenzyloxycarbonyl)-L-phenylalanylL-histidine. Deprotection of the methyl esters was performed H, CH2 (Phe) and CHI (His)), 3.95 (q,2 H, CH20),4.15-4.55 (m, in aqueous ethanol using NaOH. The crude material was re2 H, CH (Phe) and CH (His)), 7.1 and 8.35 (2 8, 2 X 1 H, 2 CH crystallized from hot acetone. The yield after crystallization (Im)), 7.2 (8, 5 H, Ph) ppm; +21.0°; 104.9. Anal. Calcd for C1&&J406 C, 57.75; H, 5.92; N, 14.96; 0,21.37. Found: C, 57.79; amounted to 65%. IR (KBr): 3300 (NH amide and carbamate), H, 5.99; N, 14.86; 0, 21.38. 1685 (C-0 carbamate), 1650 cm-' (C-0 amide), unless noted The 'H NMR spectra of the S3,S4, s6, sg, Sl0,and comotherwise. 'H NMR (methanol-d,); [aImD (c = 1.0, methanol); mp, "C: pounds were all very similar to the spectrum of S12-L-Phe-LS12-~-Ala-~-His-OH: 6 0.95 (t, 3 H, CH3), 1.3 (m, 20 H, His-OH. [ala"$+19.9', +19.7", +18.5', +18.5', +18.0', +15.9', respectively. Mp ('C): 110.1, 127.9, 135.9, 138.3, 141.2, 151.0, (CH2)10),1.4 (d, 3 H, CH3 (Ala)), 3.1 (d, 2 H, CH2(His)),3.95 (t, respectively. S3: Anal. Calcd for Cl&IUN406: C, 58.75; H, 6.23; 2 H, CH20), 4.3 (t, 1 H, CH (Ala)), 4.5 (t, 1 H, CH (His)), 7.25 N, 14.42; 0,20.60. Found C, 58.85; H, 6.29; N, 14.48; 0, 20.74. and 8.5 (2 s,2 X 1H, 2 CH (Im))ppm; +17.3'; 148.3. Anal. Calcd S:, Anal. Calcd for C&zeN40s: C, 59.69; H, 6.51; N, 13.92; 0, for C B H d 4 0 6 C, 60.25; H, 8.73; N, 12.78; 0,18.24. Found C, 19.88. Found: C, 59.78; H, 6.61; N, 13.82; 0, 19.99. Sa: Anal. 60.35; H, 8.78; N, 12.78; 0, 18.29. Cald for C&&J406 C, 61.38; H, 7.02; N, 13.01; 0,18.58. Found Sl2-~-But-~-Hie-OH (But = a-aminobutyric acid): 6 0.95 (t, C, 61.41; H, 7.22; N, 13.00, 0, 18.49. Sd Anal. Calcd for 3 H, CHS),1.0 (t,3 H, CH3 (But)), 1.3 (m, 22 H, (CH2)lo and CH2 CUHuN406: C, 62.86, H, 7.47; N, 12.22; 0,17.45. Found C, 62.71; (But)), 3.1 (d, (diet), 2 H, CH2 (His)), 3.95 (t, 2 H, CH20);4.2 (t, 1 H, CH (But)), 4.5 (t, 1 H, CH (His)), 7.25 and 8.5 (2 8, 2 X 1 H, 7.57; N, 12.22; 0,17.66. Slo: Anal. Calcd for CBHd4OS: C, 64.18; H, 7.87; N, 11.51; 0, 16.44. Found C, 64.31; H, 7.92; N, H, 2 CH (Im)) ppm; +16.3"; 131.5. Anal. Calcd for CzsH,,,N408: 11.30; 0, 16.46. s1g: Anal. Calcd for C&&&Os: C, 67.34; H, C, 61.04; H, 8.91; N, 12.38; 0, 17.68. Found: C, 61.14; H, 8.90, N, 12.40; 0, 17.65. 8.83; N, 9.82; 0,14.02. Found C, 67.19; H, 8.83; N, 9.89; 0,13.89. LPhenylalanyl-L-histidineMethyl Ester Dihydrobromide S12-~-Norval-~-His-OH: 6 0.9 (2 t, 2 X 2 H, 2 CHS),1.3 (m, ( H - L - P ~ ~ - L - H ~ ~ - O M ~(Benzyloxycarbony1)-L-phenyl.~HB~). 24 H, (CH2)loand (CH2I2(Norval)), 3.1 (d, 2 H, CH2 (His)), 4.0 alanyl-chistidine methyl ester was deproteded with HBr in glacial (t, 2 H, CH20), 4.2 (t, 1H, CH (Norval)), 4.5 (t, 1H, CH (His)), acetic acid according to a literature method." This product was 7.3 and 8.5 (2 8, 2 X 1 H, 2 CH (Im)) ppm; +16.4'; 136.9. Anal. used without further purification. The yield amounted to 98%. Cald for C a 4 0 , : C, 61.78; H, 9.07; N, 12.01; 0,17.14. Found: IR (KBr): 1740 (C=O ester), 1680 cm-' (C=O amide). 'H NMR C, 61.81; H, 9.07; N, 12.10; 0, 17.16. (methanol-d4): 6 3.1-3.6 (2 d (dist), 2 X 2 H, CH2(Phe) and CH2 S12-~-Leu-~-His-OH 6 0.9 (m, 9 H, 3 CHJ, 1.3 (m, 23 H, (His)), 3.75 ( 8 , 3 H, OCHS),4.4 (t, 1 H, CH (Phe)), 4.8 (t, 1 H, (CH2)10and CH2CH (Leu)); 3.1 (d (diet), 2 H, CH2 (His)), 4.0 (t, CH (His)), 7.3 (s,5 H,Ph), 7.4 and 8.75 (2 s, 2 X 1H, 2 CH (Im)) 2 H, CH20),4.15 (t, 1 H, CH (Leu)), 4.5 (t, 1 H, CH (His)), 7.25 ppm; +13.0°; 129.8. Anal. Calcd and 8.5 (2 s, 2 x 1H, 2 CH (Im)) PPm. N-Dodecanoyl-L-phenylalanyl-L-histidine Methyl Ester for CmH,,N406 C, 62.47; H, 9.23; N, 11.66; 0,16.64. Found C, 62.51; H, 9.23; N, 11.71; 0, 16.68. (C12-~-Phe-~-His-OMe) and N-Acetyl-L-phenylalany1-Lhistidine Methyl Ester (C1-L-Phe-L-His-OMe). H-L-Phe-LS12-t(orD)-Phe-L-His-OH 6 0.9 (t,3 H, CH3), 1.3 (m, 20 H, His-OMs2HBr was acylatd with dodecanoic anhydride or acetic (CH2)'O), 3.15 (2 d (diet), 2 X 2 H, CH2 (Phe) and CH2 (His)), 4.0 anhydride according to a literature method.16 The crude product (t, 2 H, CH20),4.45 (2 t, 2 X 1 H, CH (Phe) and CH (His)), 7.2 was diseolved in 50 mL of methanol and stirred overnight at 20 and 8.5 (2 s, 2 X 1 H, 2 CH (Im)), 7.25 (s, 5 H, Ph) ppm. L,L derivative: +17.8O; 146.1. D,L derivative: +24.7'; 143.5. Anal. 'C. The solvent was evaporated, and the crude product was subjected to column chromatography (Silica 60; chloroformCalcd for c&&O6: C, 65.35; H, 8.22; N, 10.89; 0,15.54. Found methanol, 9/1, v/v). The product was recrystallized from ethyl (LL): C, 66.31; H, 8.31, N, 10.92; 0,15.58; (D,L): C, 65.39; H, 8.23; acetate-petroleum ether. The final yield amounted to 78%. N, 10.89; 0, 15.61. C1+Phe-L-His-OMe: [ala3D -7.9' (c = 1.0, methanol). Mp: 120.3 Sl+TrpL-Hie-OH: 6 0.9 (t, 3 H, CH3),1.3 (m, 20 H, (CH&), 'C. IR (KBr): 3300 (NH amide), 1734 ( C 4 ester), 1650 cm-' 3.1 (2 d (dist), 2 X 2 H, CH2 (Trp) and CH2 (His)), 4.0 (t, 2 H, ( C = O amide). TLC (Silica): Rt = 0.45 (chloroform-methanol, CHzO),4.5 (m, 2 H, CH (Trp) and CH (His)), 7.25 and 8.45 (2 4/1, v/v). 'H NMR (chloroform-dl): 6 0.9 (t,3 H, CHs), 1.3 (m, 8, 2 X 1 H, 2 CH (Im)), 6.8-7.8 (m, 5 H, 5 CH (indolyl)) ppm; 18 H, (CH2)9),2.2 (t, 2 H, CH2CO),3.1 (2 d (dist), 2 X 2 H, CH2 +27.8'; 134.0. Anal. Calcd for C90H43Ns0s: C, 65.08; H, 7.83; (Phe) and CH2 (His)), 3.65 (e, 3 H, OCH3), 4.3-5.0 (m, 2 X 1H, N, 12.65; 0, 14.45. Found C, 65.18; H, 7.75; N, 12.65; 0,14.51. CH (Phe) and CH (His)), 6.75 and 7.55 (2 s,2 X 1 H, 2 CH (Im)), F&bPhe-bHis-OH: 6 2.7-3.3 (2 d (dist), 2 X 2 H, CH2(Phe) 7.2 (8, 5 H, Ph), 7.7 (2 d, 2 X 1 H, 2 NH (amide)), 8.9 (s (br), 1 and CH2 (His)), 4.0-4.5 (2 t (dist), 2 X 1 H, CH (Phe) and CH (His)), 5.05 (8, 2 H, CH20),7.18 (8, 5 H, Ph), 7.3 and 8.5 (2 s, 2 H, NH Um)) ppm. X 1H, 2 CH (Im)) ppm; +12.6'; 187.0; IR (KBr) 1708 cm-l (C-0 C1-tPhe-L-His-OMe: [.laOD -9.1' (c = 1.0, methanol). Mp: carbamate). Anal. Calcd for CzsHleN40$6 C, 52.48; H, 3.64; 88.3 'C. 'H NMR (methanol-d4): 6 2.0 (8, 3 H, CH3), 3.1 (m, 4 N, 10.64; 0,15.20. Found: C, 52.38; H, 3.69; N, 10.69; 0,15.16. , (s,3 H, OCHS), 4.3-4.9 (2 t (dist), H, CH2(Phe) and CH2(His))3.7 Z-L-Phe-t-His-OH: 6 3.1 (2 d (dist), 2 X 2 H, CH2 (Phe) and 2 X 1 H, 2 CHI, 6.7 and 7.4 (2 s, 2 x 1 H, 2 CH (Im)), 7.15 (e, CH2 (His)), 4.1-4.6 (2 t, 2 X 1 H, CH (Phe) and CH (His)), 4.95 5 H, C6HS) ppm. (s,2 H, CH,O), 7.15 and 8.4 (2 s, 2 X 1H, 2 CH (Im)), 7.15 (s (br), 10 H, 2 Ph) ppm; +16.5'; 205.7. Anal. Calcd for CzaHuN405: C,63.29; H, 5.54; N, 12.84; 0, 18.33. Found: C, 63.29; H, 5.59; (14) Ingles, D.W.; Knowles, J. R. Biochem. J. 1967,104, 369. N, 12.94; 0, 18.39. (15) Bodansky, M.;Vigneaud, V. J. Am. Chem. SOC.1969,81,6072. and 7.4 (2 s, 2 X 1H, 2 CH (Im)), 7.15 (8, 1H, Ph); 7.75 (d, 1H, NH (amide)), 9.0 (s (br), 1 H, NH (Im)) ppm; -6.6'; 69.0. S2-~-Phe-~-His-OMe: 6 1.1 (t, 3 H, CH3 (S2)), 3.05 (m, 2 X 2 H,CH2 (Phe) and CH2 (His)),3.6 (s,3 H,0CH3),3.9 ( q , 2 H, CHzO),4.45 (2 t (dist), 1 H, CH (Phe)), 4.8 (2 t (dist), 1H, CH (His)), 5.9 (d, 1 H, NH (carbamate)), 6.6 and 7.4 (2 8, 2 X 1 H, 2 CH (Im)), 7.5 (s,5 H, Ph), 7.5 (d, 1H, NH (amide)), 1.04 (s (br), 1 H, NH (Im)) ppm; -7.6"; 82.0. The 'H NMR spectra of the S3, S4, s6, Sg, Slo, and SI6 compounds are all very similar to the spectrum of Slz-L-Phe-L-HisOme. [alms -8.4O, -8.2", -8.1', -8.O0, -7.6O, and -7.1°, respectively. Mp (OC): 80.7, 92.4, 101.0, 109.9, 114.4, and 124.1, respectively. (Alkyloxycarbonyl)-c(or D)-X-L-histidine(&L- (or D)-XL-His-OH), (Benzyloxycarbonyl)-L-phenylalanine-Lhistidine, (Benzyloxycarbonyl)-L-alanyl-L-histidine,

Eater Cleavage by Histidine-Containing Dipeptides N-Dodecanoyl-L-phenylalanyl-L-histidine (Cl2-L-Phe-L(C1+ His-OH) and N-Acetyl-L-phenylalanyl-L-histidine Phe-L-His-OH). The methyl esters were deprotected and purified as described for the (dodecyloxycarbony1)-L-phenylalany1-Lhistidine methyl ester. The yield amounted to 68%. C1,-L-Phe-rAIis-OH: [alPD +18.5' (c = 1.0, methanol). TLc (Silica): R, = 0.3 (ethanol). Mp: 149.9 OC. IR (KBr): 3300 (NH amide), 1650 cm-' (C-0 amide). lH NMR (methanol-d4):d 0.9 (t, 3 H, CHS), 1.3 (m,18 H, (CH2)&2.15 (t, 2 H, CH20),2.7-3.3 (2 d (dist), 2 X 2 H, CH2(Phe) and CHz (His)), 4.1-4.8 (2 t (dist), 2 X 1 H, CH (Phe) and CH (His)), 7.2 and 8.3 (2 s, 2 x 1 H, 2 CH (Im)), 7.2 (s,5 H, Ph) ppm. Anal. Calcd for C&&&O4: C, 66.92; H, 8.32; N, 11.56; 0, 13.21. Found C, 67.05; H, 8.34; N, 11.66. C1-L-Phe-L-His-OH: [aImD+34.4' (c = 1.0, methanol). Mp: 240 OC dec. 'H NMR (methanol-d,): d 2.1 (8, 3 H, CHS),3.2 (2 d (dist), 2 X 2 H, 2 CH2),4.4-4.9 (2 t (dist), 2 X 1 H, 2 CH), 7.3 and 8.4 (2 s, 2 X 1 H, 2 CH (Im)),7.25 (8, 5 H, C&I4) ppm. Anal. Calcd for C1,Hd& C, 59.29; H, 5.85; N, 16.27; 0,1858. Found C, 59.01; H, 5.96; N, 16.02; 0, 18.81. N-Dodecanoyl-L-(orD)-phenylalanine 4-Nitrophenyl Ester (C12-~-(or D)-Phe-ONP). These compounds were prepared by deprotection of the Z-protected compounds1' and subsequent acylation.15 The final yield amounted to 45%. CwL-Phe-ONp: [alaOD = 10.8' (c = 1.0, chloroform);mp 108.4 OC. Anal. Calcd for Cz7HSN2O5:C, 69.21; H, 7.74; N, 5.98. Found: C, 69.31; H, 7.84; N, 5.99. C12-~Phe-ONP: +10.7O (c = 1.0, chloroform);mp 108.6 OC. Anal. Found: C, 69.33; H, 7.78; N, 5.98. IR (KBr): 3320 (NH amide); 2920 (CH stretch), 1755 (C=O ester), 1635 (C=O amide), 1525 and 1490 (NO2 stretch assym); 1347 cm-' (NO2 stretch sym). 'H NMR (CDC13): d 0.9 (t, 3 H, CH3), 1.3 (m, 18 H, (CH&, 2.2 (t, 2 H, CH2O), 3.2 (d, 2 H, CHZPh), 5.0 (2 t, 1 H, CH), 5.8 (d, 1 H, NH), 7.0 and 8.1 (2 d, 2 X 2 H, C6H4N02), 7.1 (m, 5 H, C&5) ppm. (R)- and (S)-N,N-Dimethy l-N- hexadec y l-N- (a-met hylbenzy1)ammonium Bromide (R-and S-Surf16). These compounds were prepared according to a method described in literature.16 The final yield after crystallization amounted to 44%. R compound: mp 112.0 OC; [aImD +19.g0 (c = 0.5, methanol). Anal. Calcd for C,H,NBr: C, 68.70; H, 10.64, N, 3.22; Br, 17.58. Found C, 68.78; H, 10.62; N, 3.19; Br, 17.69. S compound mp 112.3 OC; [.]?OD -19.7O (c = 0.5, methanol). Anal. Found: c, 68.72; H, 10.66; N, 3.20; Br, 17.70. 'H NMR (CDC13): 6 0.9 (t, 3 H, CH3), 1.25 (m, 28 H, (CH2)14), 1.85 (d, 3 H, CHJ, 3.2 (2 s, 2 X 3 H, 2 NCHJ, 3.5 (t, 2 H, CH2N),5.4 (9, 1 H, CHI, 7.2 (m, 5 H, C6H5) YPm. Preparation of the Surfactant Solutions. Tris(hydroxymethyllaminomethane (Baker) and potassium chloride (Baker) were dissolved in double distilled water. The concentrations amounted to 0.08 and 0.40 M, respectively. The pH was adjusted to 7.3 with the aid of concentrated HCl (Merck). The surfactant was dissolved in this buffer to a concentrationof 2.5 or 5.0 X lo" M. The buffered surfactant solution was divided into two parts. (16) (a) Conti, C. Biochem. Biophys. Res. Commun. 1974,57,1287. (b) Walker, M.S . J . Chem. Phys. 1967,47,1020. (c) Eftink, M. R.; Ghiron,

C. A. Arch. Biochem. Biophys. 1981,209,706. (d) Eefahani, J. J. Biol. Chem. 1982,257,9919.

J. Org. Chem., Vol. 56, No. 12, 1991 3891 One part was used to obtain the blank reaction r a t a in the abeence of catalyst. To the other part the finely powdered catalyst was added (5 X lob M) and the solution was stirred for 2 h at 40 O C in a sealed flask. The thus obtained solution was used to determine the reaction rates in the presence of catalyst. It was checked separately that sonication of the buffered catalystsurfactant solutions had no effect on the observed rates. Therefore, sonication was ommited. Kinetic Measurements. A UV cell containing 2.9 mL of the buffered surfactant solution (with or without catalyst) was placed in a UV/vis spectrophotometer thermostated at 25 OC. The reaction was started upon the injection of the substrate, which was dissolved in 0.1 mL of acetonitrile (Baker). The final substrate M. The release of the concentration amounted to 1.0 X 4-nitrophenolate ion was followed by the increase in absorption at 400 nm. The rate data obeyed a pseudo-firsborder rate profile, and the rate constants were calculated as the average value obtained from four repeated runs. The second-order rate constants, were obtained with the aid of the following formula: k w b = k , - kbl, in which k , is the second-order rate constant measured in the presence of catalyst and kbl is the second-order rate constant measured in its absence (blank or background reaction). The estimated error in k,,b amounts to 5%. Registry No. S12C1, 24460-74-0; ZC1, 501-53-1; p-BrZC1, 5798-78-7; F5ZCl, 53526-74-2; SIC1, 79-22-1; S2C1,541-41-3; Ala, 56-41-7;But, 1492-24-6; Nva, 66oo-10-4;Leu, 61-90-5; Phe, 63-91-2; Trp, 73-22-3; S12-Ala-OH,133230-62-3;S12-But-OH,133230-63-4; S12-Nva-OH,133230-64-5;S12-Leu-OH,133230-65-6; S12-Phe-OH, 133230-66-7; S12-Trp-OH,133230-67-8; Z-Phe-OH, 1161-13-3; p-BrZPhe-OH, 40297-81-2;F&Phe-OH, 133230-68-9; %Ala-OH, 1142-20-7;S1-Phe-OH,41844-91-1; S2-Phe-OH,19887-32-2;HisOMe2HC1, 7389-87-9; S12-Ala-His-OME,133230-69-0;S12-ButHis-OMe, 133230-70-3;Sz2-Nva-His-OMe,133230-71-4;S12-LeuHis-OMe, 133230-72-5; Slz-Phe-His-OMe, 133230-73-6; slz-DPhe-His-OMe, 133230-74-7; Slz-Trp-His-OMe, 133230-75-8; ZPhe-His-OMe, 16689-13-7; F5Z-Phe-His-OMe, 133230-76-9; p BrZ-Phe-His-OMe, 133230-77-0; Z-Ala-His-OMe, 32303-82-5; S1-Phe-His-OMe, 133230-78-1; S2-Phe-His-OMe, 133230-79-2; S12-Ala-His-OH,133230-80-5; S12-But-His-OH, 133230-81-6; S2,-Nva-His-OH, 133230-82-7; Slz-Leu-His-OH, 133230-83-8; S12-Phe-His-OH,133230-84-9;S12-~-Phe-His-OH, 133230-85-0; Slz-Trp-His-OH, 133230-86-1; F5Z-Phe-His-OH, 133230-87-2; Z-Phe-His-OH, 20806-38-6; p-Brz-Phe-His-OH, 133230-88-3; Z-Ala-His-OH, 79458-92-7; S1-Phe-His-OH, 133230-89-4; SzPhe-His-OH, 114346-47-3; Phe-His-OMe-aHBr, 18779-16-3; (HsC(CH2)loC0)20,645-66-9; Clz-Phe-His-OMe, 79416-20-9; C1-Phe-His-OMe, 133230-90-7; C12-Phe-His-OH,90703-14-3; C1-Phe-His-OH, 123580-40-5;C12-Phe-ONP,75531-11-2; clz-DPhe-ONP, 75531-12-3;R-sI.u~16,50640-92-1;S-surf 16,50640-91-0; S3-Phe-OH, 85590-63-2; S,-Phe-OH, 75048-11-2; S6-Phe-OH', 133230-91-8;S8-Phe-OH, 133230-92-9;Slo-Phe-OH,133230-93-0; S16-Phe-OH, 133230-94-1; S3-Phe-His-OMe, 133230-95-2; s4Phe-His-OMe, 133230-96-3; S6-Phe-His-OMe,133230-97-4; 8sPhe-His-OMe, 133230-98-5; Slo-Phe-His-OMe, 133230-99-6; S16-Phe-His-OMe,133231-00-2; SS-Phe-His-OH, 133231-01-3; S4-Phe-His-OH,133231-02-4;S6-Phe-His-OH,133231-03-5; SSPhe-His-OH, 133231-04-6; Slo-Phe-His-OH, 133231-05-7; SlePhe-His-OH, 133231-06-8; ZPhe-ONP, 2578-84-9; ZDPhe-ONP, 2578-85-0.